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通过多重反应监测鉴定临床样本中前列腺特异性抗原的新型蛋白水解产物 (SNP-L132I)。

Identification of a novel proteoform of prostate specific antigen (SNP-L132I) in clinical samples by multiple reaction monitoring.

机构信息

Clinical Protein Science & Imaging, Biomedical Center, Dept. of Measurement Technology and Industrial Electrical Engineering, Lund University, BMC C13, 221 84 Lund, Sweden;

出版信息

Mol Cell Proteomics. 2013 Oct;12(10):2761-73. doi: 10.1074/mcp.M113.028365. Epub 2013 Jul 10.

Abstract

Prostate specific antigen (PSA) is a well-established tumor marker that is frequently employed as model biomarker in the development and evaluation of emerging quantitative proteomics techniques, partially as a result of wide access to commercialized immunoassays serving as "gold standards." We designed a multiple reaction monitoring (MRM) assay to detect PSA proteoforms in clinical samples (n = 72), utilizing the specificity and sensitivity of the method. We report, for the first time, a PSA proteoform coded by SNP-L132I (rs2003783) that was observed in nine samples in both heterozygous (n = 7) and homozygous (n = 2) expression profiles. Other isoforms of PSA, derived from protein databases, were not identified by four unique proteotypic tryptic peptides. We have also utilized our MRM assay for precise quantitative analysis of PSA concentrations in both seminal and blood plasma samples. The analytical performance was evaluated, and close agreement was noted between quantitations based on three selected peptides (LSEPAELTDAVK, IVGGWECEK, and SVILLGR) and a routinely used commercialized immunoassay. Additionally, we disclose that the peptide IVGGWECEK is shared with kallikrein-related peptidase 2 and therefore is not unique for PSA. Thus, we propose the use of another tryptic sequence (SVILLGR) for accurate MRM quantification of PSA in clinical samples.

摘要

前列腺特异性抗原(PSA)是一种成熟的肿瘤标志物,常用于新兴定量蛋白质组学技术的开发和评估中,部分原因是广泛使用商业化的免疫测定作为“金标准”。我们设计了一种多重反应监测(MRM)测定法来检测临床样本中的 PSA 蛋白形式(n = 72),利用该方法的特异性和灵敏度。我们首次报告了一种由 SNP-L132I(rs2003783)编码的 PSA 蛋白形式,在 9 个样本中以杂合子(n = 7)和纯合子(n = 2)的表达谱观察到。来自蛋白质数据库的其他 PSA 同工型无法通过四个独特的肽酶切肽识别。我们还利用我们的 MRM 测定法对精液和血浆样本中的 PSA 浓度进行精确的定量分析。评估了分析性能,并注意到基于三个选定肽(LSEPAELTDAVK、IVGGWECEK 和 SVILLGR)和常规使用的商业化免疫测定的定量之间存在密切的一致性。此外,我们披露肽 IVGGWECEK 与激肽释放酶相关肽酶 2 共享,因此并非 PSA 所特有。因此,我们建议在临床样本中使用另一种胰蛋白酶序列(SVILLGR)进行 PSA 的准确 MRM 定量。

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